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Munc13 非依赖性囊泡引发小鼠光感受器突触上的带状突触

Munc13-independent vesicle priming at mouse photoreceptor ribbon synapses.

机构信息

Department of Molecular Neurobiology, Max Planck Institute of Experimental Medicine, D-37075 Göttingen, Germany.

出版信息

J Neurosci. 2012 Jun 6;32(23):8040-52. doi: 10.1523/JNEUROSCI.4240-11.2012.

Abstract

Munc13 proteins are essential regulators of exocytosis. In hippocampal glutamatergic neurons, the genetic deletion of Munc13s results in the complete loss of primed synaptic vesicles (SVs) in direct contact with the presynaptic active zone membrane, and in a total block of neurotransmitter release. Similarly drastic consequences of Munc13 loss are detectable in hippocampal and striatal GABAergic neurons. We show here that, in the adult mouse retina, the two Munc13-2 splice variants bMunc13-2 and ubMunc13-2 are selectively localized to conventional and ribbon synapses, respectively, and that ubMunc13-2 is the only Munc13 isoform in mature photoreceptor ribbon synapses. Strikingly, the genetic deletion of ubMunc13-2 has little effect on synaptic signaling by photoreceptor ribbon synapses and does not prevent membrane attachment of synaptic vesicles at the photoreceptor ribbon synaptic site. Thus, photoreceptor ribbon synapses and conventional synapses differ fundamentally with regard to their dependence on SV priming proteins of the Munc13 family. Their function is only moderately affected by Munc13 loss, which leads to slight perturbations of signal integration in the retina.

摘要

Munc13 蛋白是胞吐作用的重要调节因子。在海马谷氨酸能神经元中,Munc13s 的基因缺失导致与突触前活性区膜直接接触的已成熟突触小泡 (SVs) 完全丢失,并完全阻断神经递质释放。在海马和纹状体 GABA 能神经元中也可检测到 Munc13 缺失的类似严重后果。我们在这里表明,在成年小鼠视网膜中,两种 Munc13-2 剪接变体 bMunc13-2 和 ubMunc13-2 分别选择性地定位于常规和带状突触,并且 ubMunc13-2 是成熟光感受器带状突触中唯一的 Munc13 同工型。令人惊讶的是,ubMunc13-2 的基因缺失对光感受器带状突触的突触信号传递几乎没有影响,并且不会阻止突触小泡在光感受器带状突触部位的膜附着。因此,光感受器带状突触和常规突触在其对 Munc13 家族的 SV 引发蛋白的依赖性方面存在根本差异。它们的功能仅被 Munc13 缺失适度影响,这导致视网膜中信号整合的轻微扰动。

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本文引用的文献

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Molecular organization and plasticity of the cytomatrix at the active zone.活性区细胞基质的分子组织和可塑性。
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